Upload
others
View
2
Download
0
Embed Size (px)
Citation preview
Vol. 7, 397-403, May 1998 Cancer Epidemiology, Biomarkers & Prevention 397
p53 Mutations in Cyclophosphamide-associated Bladder Cancer
Mohammed A. Khan, Lois B. Travis, Charles F. Lynch,Ylermi Soini, Andrew M. Hruszkewycz,Rosario M. Delgado, Eric J. Holowaty,Flora E. van Leeuwen, Bengt Glimelius, Marilyn Stovall,John D. Boice, Jr., Robert E. Tarone, andWilliam P. Bennett’
Laboratory of Human Carcinogenesis [M. A. K.]. Radiation Epidemiology
Branch, Division of Cancer Epidemiology and Genetics [L. B. T., J. D. B.l,
Biostatistics Branch, Division of Cancer Epidemiology and Genetics [R. E. TI,
National Cancer Institute, and Clinical Pathology Department, Clinical Center
[A. M. H., R. M. Dl, NIH. Bethesda, Maryland 20892; Department of
Preventive Medicine and Environmental Health, University of Iowa, Iowa
City, Iowa 52242 [C. F. LI; Department of Pathology, Central University
Hospital, University of Oulu, Oulu, SF-90220, Finland [Y. S.]; Department of
Pathology. Central University Hospital. University of Tampere, Tampere,
Finland [Y. 5.1; Ontario Cancer Treatment and Research Foundation, Toronto,
Ontario, M5G-2L7, Canada [E. J. HI; Netherlands Cancer Institute,
Amsterdam. 1066-CX, The Netherlands [F. E. V. L.]; Department of Oncology,
University Hospital. Uppsala, 5-751-75, Sweden [B. G.l; University of TexasM. D. Anderson Cancer Center, Houston. Texas 77030 IM. 5.1; and Division
of Human Genetics. City of Hope National Medical Center, Duarte, California
91010 [W.P.B.I
Abstract
Cyclophosphamide is a known bladder carcinogen, withcumulative dose directly related to increased risk. Thereis no consensus, however, on which majorcyclophosphamide metabolite (i.e., acrolein orphosphoramide mustard) drives bladder carcinogenesis.We examined 19 cyclophosphamide-related bladdertumors to test the hypothesis that they might containsomatic mutations in the p53 tumor suppressor gene thatcould link a specific metabolite to the etiology of thesecancers. Forty-three % (9 of 19) of the cases had amutation in p5.3, with a predominance at G:C bp (7 of 9,77%), a preference for non-CpG sites (6 of 7, 86%), andfrequent G:C-s�A:T transitions (5 of 7, 71 %). The p53mutation spectrum of these cyclophosphamide-associatedbladder cancers differed significantly from patternsreported for sporadic (P 0.020), smoking-related
(0.043), and schistosomiasis-linked (P 0.002) tumorsbut not arylamine-associated neoplasms (P = 0.860).
Differences between the cyclophosphamide andarylamine-associated spectra included an unusual degree
of clustering of exon 6 mutations (43% versus 17%,respectively) and an absence of multiple mutations in theformer. Notably lacking in our series were G:C-�T:Atransversions, the principal mutation associated with
Received I 1/2 1/97; revised 2/I 3/98; accepted 2/26/98.
The costs of publication of this article were defrayed in part by the payment of
page charges. This article must therefore be hereby marked advertisement in
accordance with 18 U.S.C. Section 1734 solely to indicate this fact.
I To whom requests for reprints should be addressed, at Division of Human
Genetics, City of Hope National Medical Center. Fox Plaza South. 2nd Floor.1500 E. Duarte Road. Duarte, CA 91010-3000. Phone: (626) 256-8726; Fax:
(626) 301-8142: E-mail: [email protected].
acrolein. Instead, the mutation spectrum matches thephosphoramide mustard adduction sequences determinedby a repetitive primer-extension assay (P = 0.024),
indicating that this metabolite might be a key mutagen incvelonhosnhamide-related bladder cancer.
Introduction
Cyclophosphamide is a known bladder carcinogen with a
highly significant relationship between cumulative dose andbladder cancer risk ( 1 ). This cytotoxic agent is prescribed to
500,000 patients each year worldwide (2), and the resultingbladder cancers may have both early onset and an aggressivecourse (3). Although three major, DNA-binding metabolites(phosphoramide mustard, nornitrogen mustard, and acrolein;Fig. lA) result from the metabolism of cyclophosphamide by
mixed function oxidases, there is no consensus on which prod-uct drives bladder carcinogenesis. Many investigators consider
the primary mutagen to be phosphoramide mustard (4-6), whichforms monofunctional and bifunctional guanine adducts (7); nor-
nitrogen mustard may also play a role because it has similar
chemical properties (Ref. 7; Fig. IB). Acrolein is mutagenic inanimal models (4, 5, 7, 8) and human cells in vitro (9, 10), but itis not a proven carcinogen, possibly because of its extreme toxicity
(1 1). Clinical data correlating acrolein-induced hemorrhagic cys-titis with subsequent bladder cancer is conflicting ( I 2-14). Giventhe uncertainty over the role of acrolein as a bladder carcinogen,we evaluated a series of bladder cancers which followed cyclo-phosphamide therapy (1) to test the hypothesis that patterns of
somatic mutations might link acrolein, phosphoramide mustard, ornomitrogen mustard to the etiology of these cancers. We tested for
mutations in the p53 tumor suppressor gene because it plays aprominent role in the development of bladder cancer (reviewed inRef. I 5) and because characteristic mutational spectra have been
reported for two other bladder carcinogens, tobacco ( I 6) and
schistosomiasis (17).
Materials and Methods
Study Population. All available tissue samples were obtainedfrom a case-control study of secondary bladder cancer ( I)
conducted within a cohort of 6171 2-year survivors of non-Hodgkin’s lymphoma (18). In this analytic investigation, which
represents the largest study to date of cyclophosphamide-asso-ciated bladder cancer, the relative risk associated with cumu-lative doses ofcyclophosphamide <20, 20-50, and >50 g were2.4, 6.3, and 14.5, respectively (P-trend = 0.004; Ref. 1). With
the approval of local boards governing research on humansubjects, resection or biopsy tissues were requested for all
patients in the case-control study, with specimens available for19 primary bladder cancers from 18 patients. The second blad-
der cancers occurred an average of I 2 years after lymphomadiagnosis. Data on cumulative cyclophosphamide dose, radia-tion dose to bladder, interval between lymphoma and bladder
cancer, and other pertinent clinical information for the I 8patients are summarized in Table I . All subjects were treated
Association for Cancer Research. by guest on October 8, 2020. Copyright 1998 Americanhttps://bloodcancerdiscov.aacrjournals.orgDownloaded from
A /-3L�c::#{176}c�1 P455
,.- 4-
\-� aCyclophosphamide
Ozidase
EnzymaflcInactivation
+H�L�
Acrolein
B
Phosphoramide Mustard
Phosphoramide Mustard DNA Adducts:
2
nor-C-OH
,o�2
nor-C
NH 2 3’-dGMP-Pho!phoesterAdduct
C-nor-C
Nornitrogen Mustard DNA Adduct:(O,S,N)-protein
2
7, 8-Cyclic Cuanine Adduct
N�’�
398 p53 in Cyclophosphamide-linked Cancer
Carboxyphosphamide
�Cl
�Cl
Nornitrogen Mustard
Acrolein DNA Adducts:
6-Hydroxy-1,N2-PropanodG
S.Hydroxy-l, N2-PrapanodG
OH 0
Fig. 1. A, metabolism of cyclophosph-
amide to phosphoramide mustard, acro-1cm, and nornitrogen mustard. Cyclo-
phosphamide is metabolized by
cytochrome P450 enzymes to 4-hy-
droxycyclophosphamide, which equili-
brates with aldophosphamide to sponta-
neously yield phosphoramide mustard
and acrolein. Aldophosphamide is also
metabolized by aldehyde oxidase to car-
boxyphosphamide, which produces nor-
nitrogen mustard. 4-Hydroxy-cyclo-
phosphamide can be oxidized to theinactive 4-keto-cyclophosphamide. B.
phosphoramide mustard produces mul-
tiple monofunctional and bifunctional
adducts with guanine. and acrolein
forms exocyclic adducts. Nornitrogen
mustard forms mono- and bifunctional
adducts with guanine. Figure adapted
from Anderson et a!. (5) and Povirk and
Shuker (7).
with cyclophosphamide (median cumulative dose, 16.6 g;
range, 6-125.2 g), and some also received radiotherapy.
Genomic DNA Extraction, p53 PCR Amplification, andDNA Sequence Analysis. Tumor and nontumor tissues weremicrodissected from unstained, paraffin-embedded, formalin-
fixed histological sections. After proteinase K digestion,
genomic DNA was isolated by organic extraction as described(19). Exons 5-8 were amplified individually using nested prim-
ers, and each product was sequenced as reported previously(19); mutations were confirmed by finding the same base
change in two independent PCR products.
Statistical Analyses. The overall type and distribution of mu-tations among the 570 bp in exons 5-8 of the p53 gene in the
cyclophosphamide-associated bladder cancers were compared
with the mutational spectra observed in sporadic bladder can-
cers and those linked to tobacco use, schistosomiasis, and arylam-
me exposure using the procedure described by Cariello et a!. (20).
This method uses the Adams and Skopek algorithm to estimate P
corresponding to an exact multivariate hypergeometric test for
contingency tables (21). A random number generator simulates a
large number of spectra based on the multivariate hypergeometric
distribution, conditional on the numbers and locations of mutations
in the two series to be compared.
The frequency of specific mutations within p53 exons was
compared with the distribution reported for bladder cancers
following exposure to other known carcinogens or to sporadic
Association for Cancer Research. by guest on October 8, 2020. Copyright 1998 Americanhttps://bloodcancerdiscov.aacrjournals.orgDownloaded from
Table I Secondary bladder cancer after cyclophosphamide therapy for non-Hodgkin’s lymphoma: Patient summaries and p53 analyses
Non-Hodgkin’s lymphoma Bladder cancer p53 sequence analysis
Patient
no-
Age” (yr)/
SexTobacco usc5
NHL DX’ NHL All
(mo/yr) stage therapy
Begin-End
(mo/yr)
Total
dose ofCIX”
(g)
Total
radiation
dose to
bladder
(Gy)
Interval NHL to
bladder cancer
(yr)IhistologyCodon:Mutation Base
change
CpG
site
34.7 13.5IFCC WT1 671M Ex-smoker 1/74 Unk CVP 1/78-12/78 24.0
RT 11/77-12/77
2 62/M 5 cigars/day 1 1/78 II RT 12/78-1/79 13.5 33.8 5.5/TCC WT
RT 1/79-1/79
CVP 2/79-5/79
CHVP 5/79-2/80
RT 3/80-3/80
RT 5/80-5/80
RT 10/80-10/80
3 58/M Ex-smoker. < 1 PPD 6/77 II RT 7/77-8/77 8.8 <0. 1 lO.0/TCC WT
CVP 1/78-6/78
4 64/F None 3/69 III RT 4/69-4/69 34.0 6.5 14.2/Pap. TCC WT
CTX 10/69-10/71
5 6I/M Pipe-smoker. heavy 1/75 IV CVP 2/75-7/75 10.3 19.5 6.1ITCC 230: ACC’5’-ATC’� G:C-’A:T No
RT
RT
RT
RT
1/75-1/75
8/75-9/75
10/75-11/75
12/75-1/76
6 6l/M >2 PPD X 40 yr 12/70 III RT 1/71-1/71 47.2 5.4 6.4/SqCC 279: GGG�-�AGG’� G:C-’A:T No
COPP
ABVD
RT
11/72-3/77
3/77-4/77
5/76-6/76
7 691M Ex-smoker. cigarette/
pipe
7/78 Unk BACOP
RT
1/84-7/84
1/79-1/79
13.3 <0. 1 7.2/Pap. TCC WT
8 681M Ex-smoker, other
tobacco
10/78 Unk CTX
COPP
RT
1 1/78-4/79
4/79-5/80
3/79-4/79
20.2 <0. 1 3.9/Pap. TCC 241 : TCC�’-iACC�” A:T-.T:A NA
9 65/M Ex-smoker 1-2 PPD 3/78 I CHOP
RT
6/78-12/78
5/78-6/78
6.0 38.8 6.3iTCC WT
10 46/M >2 PPD 2/79 Unk CHOP 3/80-1 1/80 56.0 (None) 5.9/TCC 261’: AG-*AA G:C-’A:T No
MEV-LMTX
1 1/80-5/82
1 1 67/F None 2/74 I COPP 6/74-5/76 12.0 23.8 1 1.5/Pap. ICC 199: GGA�-’AGA�� G:C-*A:T No
RT 4/74-5/74
l2� 6l/M Ex-pipe 7/84 IV RT 7/84-7/84 15.3 0.9 3.4/Pap. TCC WT
BACOP 7/84-1/85
1Y 63/M Cigars 1/79 III COPP 2/79-8/79 49.6 17.3 12.3/Pap. ICC 193: � A:T-.G:C NA
RT
COPP
8/79-9/79
2/80-4/84
l4� 56/F 1-2 PPD 4/81 IV CHOP 5/81-1 1/82 18.0 (None) 8.7/Pap. TCC WT
l5� 38/M 1-2 PPD 12/78 IV CHOP 12/78-9/79 125.2 (None) 10.811CC WT
CTX
CHLB
C.rxVLB
MTX
9/79-9/82
9/82-3/83
3/83-1/85
1/85-12/85
12/85-1/90
l6�� 52/M 2 PPD x 36 yr 10/83 II or
lIla
CHOP I 1/83-3/84 8.3 (None) 6.6/Pap. TCC 196: �
188: CTG”-GTG�”1
G:C-iC:G
G:C-iC:G
Yes
No
17’ 67/F None 6/81 II CHOP 7/81-12/81 6.4 (None) 5.7/Pap. TCC WT
1W 61/M 1-2 PPD X 50 yr 8/79 IV CHOP 8/79-12/79 30.5 (None) 12.8/Pap. TCC 135: TGCcy��*TACvr G:C-*A:T No
CTX 12/79-4/82
C, At diagnosis of non-Hodgkin’s lymphoma.b All histories refer to cigarette use unless noted otherwise.‘. DX, diagnosis; ABVD, doxorubicin, bleomycin, vincristine, and dacarbazine; BACOP, cyclophosphamide. bleomycin, doxorubicin, vincristine, and prednisone: CDDP,
cisplatin; CHLB, chlorambucil; CHOP, cyclophosphamide, doxorubicin, vincristine, and prednisone; CHVP, cyclophosphamide, doxorubicin, teniposide. and prednisone:
COPP, cyclophosphamide, vincristine, procarbazine, and prednisone; CTX, cyclophosphamide; CVP, cyclophosphamide, vincnstine, and prednisone; IMTX. intrathecal
methotrexate; MEV, cyclophosphamide, methotrexate, and vincristine; NA, not applicable; NHL, non-Hodgkin’s lymphoma; Pap. TCC, papillary transitional cell
carcinoma; PPD, pack(s) per day; RT, radiotherapy; SqCC, squamous cell carcinoma; TCC, transitional cell carcinoma; Unk, unknown; WT, wild type.
d Cumulative dose of cyclophosphamide.
� The mutation in Patient 10 occurred in the 5’ splice site for exon 8 adjacent to the last nucleotide of codon 261.
‘�Case was not included in the prior analytic investigation (1) because strict eligibility criteria were not met or because the bladder cancer developed after the close of
follow-up (December 31, 1989).g Patient 16 had a second bladder cancer diagnosed 9.6 years after the NHL.
Cancer Epidemiology, Biomarkers & Prevention 399
Association for Cancer Research. by guest on October 8, 2020. Copyright 1998 Americanhttps://bloodcancerdiscov.aacrjournals.orgDownloaded from
40’.) p53 in Cyclophosphamide-linked Cancer
Table 2 p53 mutatio n spectra in hum an bladd er cancers linked to cyclophosphamide therapy. occupat
known exposures (i.e.. sporadic)
ional cx posure to arylamin e. schistosomi axis, smoking. or no
Exposure beforebladder cancer
Mut. Freq.”(%(
i,,,G:C-
AT AT. . T:A C:G(CpG) (non-CpG)
G:C
A:T-*
T.A C:G
Del/lns/
Other
Mutations in
exon 6
% P
Cyclophosphamide
Arylarnine
Schistosomiasis
Tobacco
Sporadic”
49
47
40
NA
34
9
27
71
81
113
NA
0.860
0.002
0.043
0.020
0 5 0 2
0 17 3 1
21 20 7 9
9 32 9 14
18 24 16 18
1
4
6
3
II
1
1
2
1
5
0
0
0
5
5
0
1
6
7
16
44 NA
17 0.300
10 0.045
10 0.044
6 0.012
“ Mut. Freq., mutation frequency; NA. not applicable.
I, Comparison of the overall p53 mutation spectrum in cyclophosphamide-associated tumors with those observed in the indicated series. Data for sporadic. schistosomiasis,
tobacco. and arylaminc-associated bladder cancers were collected from the p53 mutation database (54) and compared with the cyclophosphamide spectrum by Monte Carlo
analysis (Ref. 20; see ‘Materials and Methods” for additional description). Statistically significant (P < 0.05) differences were observed between the pattern of p53
mutations in cyclophosphamide-associated cases compared with sporadic. schistosomiasis. and tobacco-related tumors.
‘ The cyclophosphamide-linked p53 mutations clustered in exon 6 (44%) were compared with other bladder cancer series, and the differences were statistically significant
for all comparisons except arylamine (Fisher’s exact test, two-tailed), with Ps denoted in this column. p53 mutations occurring in exons 5-8 in sporadic bladder cancers
and those linked to schistosomiasis, tobacco, and arylamine were retrieved from the p53 mutation database (54).
,‘ The I I 3 mutations from “sporadic” tumors exclude all other groups.
cases by means of the two-tailed Fisher’s exact test. An exact
permutation test for trend (2 1 ) was conducted to test for adose-response between cumulative amount of cyclophospha-mide and p53 mutations. Exact binomial Ps were calculated totest whether a significant excess of mutations or adducts oc-curred within a selected class of nucleotides.
Results
p53 Mutations. Nine p53 mutations occurred in 8 of 18 pa-
tients with secondary bladder cancer. Patient 16 had two blad-der cancers that were diagnosed 3 years apart and containeddifferent p53 mutations; due to the time interval, disparatemutations, and established precedent (22, 23), these were con-sidered as separate, metachronous tumors (i.e., not metastatic orrecurrent lesions). The nine mutations consisted of five
G:C-s’A:T transitions (all non-CpG sites), two G:C-*C:Gtransversions (one CpG and one non-CpG site), one A:T-*T:A
transversion, and one A:T-*G:C transition (Table I ). Distri-bution by exon was as follows: one (I 1%) in exon 5, 4 (45%)
in exon 6, two (22%) in exon 7, and two (22%) in exon 8.
The Cyclophosphamide Mutation Spectrum Is Distinctamong Bladder Cancers and Concentrates in Exon 6. Theoverall p53 mutation spectrum in cyclophosphamide-associated
tumors differed significantly from those described in sporadic(P = 0.020), smoking-related (P 0.043), and schistosomia-
sis-associated (P 0.002) bladder cancer but not arylamine-linked cancers (P = 0.86). The predominant mutations in ourseries were G:C-�A:T transitions occurring only at non-CpGsites (five of five), similar to mutations described for arylamine.In contrast, ratios of G:C>A:T transitions at non-CpG versus
CpG sites for most other bladder cancer series varied from I :1(schistosomiasis) to 1 :4 (tobacco).
Cyclophosphamide-associated bladder cancers differedmarkedly from those related to arylamine in the degree ofmutational clustering in exon 6 and in the absence of multiple
lesions. Four (44%) of the nine mutations in our study and three(43%) of the seven mutations at G:C bp occurred in exon 6, adisproportionate representation, given the small size of thisexon (37 codons) compared with exons 5, 7, and 8 (142 codons).Moreover, the percentage of mutations in exon 6 in cyclophosph-amide-associated tumors was considerably larger than the fre-
quency (6-17%) reported for sporadic bladder cancers (P -
0.012) or those linked to tobacco (P = 0.044), schistosomia.sis
(0.045), or arylamine (P = 0.30, see Table 2). Multiple p53
mutations, which were not observed in our series, were prominentin bladder malignancies after arylamine exposure (24).
Investigation of a Possible Dose-Response Relationship be-tween Cyclophosphamide and p5.3 Mutation Rates. Muta-tions at G:C bp in non-CpG sites (n = 6) were categorized
according to cyclophosphamide dose groups used in the anal-ysis of the prior case-control study ( 1 ); 27% (3 of I I ), 33% (2
of 6), and 50% (1 of 2) occurred in the <20-, 20-50-, and>50-g groups, respectively (P = 0.40). A similar pattern was
observed when all p53 mutations were analyzed according to
cumulative cyclophosphamide dose categories (P 0.31).
Discussion
Cyclophosphamide Produces a Mutation Spectrum ThatMatches Phosphoramide Mustard Adduction Sites. Weprovide the first description of p.53 mutations in cyclophosph-amide-related bladder cancers. The p53 mutation spectrum in
these tumors is distinguished by a predominance of mutationsat G:C bp, a preference for non-CpG sites, an excess of
G:C>A:T transitions, and a clustering in exon 6. This unusualconstellation of features differs significantly from sporadic,smoking-related, and schistosomiasis-linked bladder cancers,
and the concentration of mutations in exon 6 differs markedlyfrom bladder tumors in these series (Table 2). The character andlocation of mutations in cyclophosphamide-related bladder can-cer match the distribution of phosphoramide mustard adductsdetermined by a repetitive primer-extension assay (25). Boththe mutations and the adducts have strong preferences for G:C
bp at non-CpG dinucleotides, with significant excesses of p53mutations and strong adduct sites in exon 6. Furthermore, three(43%) of seven mutations at G:C bp in our series occupiedstrong adduct sites. It is unlikely that this distribution occurred
by chance alone (P = 0.018, binomial probability), becauseonly 6.8% of G:C pairs are found at these locations. Taken
together, our data suggest that phosphoramide mustard may bean important mutagenic metabolite in cyclophosphamide-re-lated bladder cancer.
Phosphoramide Mustard Forms Guanine Adducts withinConsensus Sequences. Phosphoramide mustard and nornitro-gen mustard form adducts predominantly at the N7-position of
guanine, occasionally at the N3 position of cytosine (reviewedin Refs. 5, 7, and 8), and rarely at adenine or thymidine (26, 27).
Association for Cancer Research. by guest on October 8, 2020. Copyright 1998 Americanhttps://bloodcancerdiscov.aacrjournals.orgDownloaded from
241
248
158
183
196
iiiliiiniihiiiiiiiIiiillilIi/‘
--- -_�&�
Cancer Epidemiology, Biomarkers & Prevention 401
6(05C0
*1 #{149}
0 liii I III
Strong Adduct Sites Mutations at G:C Base Pairs: I Sporadic
� Cyclophosphamide
Fig. 2. Distribution of cyclophosphamide-induced p53 mutations compared with mutations from sporadic tumors and adduction sites for phosphoramide mustard. The
p53 coding sequences for exons 5-8 are represented by the horizontal bar. The cyclophosphamide-linked mutations (yellow columns with diamonds) and sporadic mutations
(black columns) are shown. The locations of phosphoramide mustard adducts were determined by a repetitive primer-extension analysis of human alphoid DNA (25). and
the consensus sequences for strong adducts are indicated by yellow triangles.
Consensus sequences flanking preferential guanine adductionsites were recently defined by a repetitive primer extensionassay (25) used to map the location and intensity of DNA
adducts in human cells. These experiments found phosphor-
amide mustard adducts only at guanine residues, as reportedpreviously (26, 27). There were variations in binding intensityamong guanines, and consensus sequences for strong, interme-diate, and weak adduction sites were defined; it is notable thatadduction of guanines flanked by cytosine was rare (25). Be-
cause acrolein adducts are not detected by this assay (25), the
adducts were produced either by phosphoramide mustard ornornitrogen mustard. When these consensus sequences arecompared with p53 coding regions, there is a striking clustering
of strong adduction sites in exon 6 (n = 9) compared with exon
8 (n 6) or exons 5 and 7 (n 3 each; Fig. 2). It is unlikely
that 9 (43%) of 21 strong adduct sites occurred in exon 6 bychance (P = 0.024, binomial probability), because this exoncontains only 19.4% of G:C sites. Nornitrogen mustard may alsobe a plausible mutagen, but we cannot assess the contribution ofthis metabolite until its associated adduct distribution has beendetermined.
Phosphoramide Mustard Adducts Match Cyclophospha-mide-induced p5.3 Mutations. All major features of the phos-
phoramide mustard adduct distribution are seen in the p.53
mutations, including a strong preference for non-CpG sites anda notable exon 6 clustering. In fact, cogent arguments link allseven mutations at G:C bp in our series to phosphoramide
mustard adducts. For example, all matched strong (3), interme-diate (I ), or weak (3) consensus adduction sequences and all
but two of the mutation sites had at least 80% homology to theconsensus adduction sequences (Ref. 25; Table 3). Five ofseven mutations at G:C bp have a coding strand bias, which ischaracteristic of chemical carcinogens due to preferential repair
of the transcribed strand (28, 29); it is notable that the twoexceptions (i.e., patients S and 16) occupy strong adduction
sites that may compensate for the rapid repair of the transcribedstrand. Data for DNA repair rates within the p53 coding se-
quences are incomplete, but three ofthe mutations (i.e., patients6, 13, and 16) occupy known slow spots for DNA repair, whichis a predisposing factor for mutation (30).
DNA-adduct hotspots were previously linked with char-acteristic mutations in a report correlating the distribution ofp53 mutations in human lung cancer with the DNA adductdistribution of benzo(a)pyrene diol-epoxide, a carcinogen in
tobacco smoke (31). Our study provides the first exampledescribing homology of carcinogen-DNA adduct hotspots
with the pattern of p.53 mutations in an iatrogenic cancer.There are no reports, to our knowledge, of the mutation
spectrum generated by cyclophosphamide in animal or in
vitro models.
Acrolein: Toxicity, Adducts, and Mutation Spectrum. Dc-spite the established role of acrolein in hemorrhagic cystitis(14), there is insufficient evidence to classify it as a carcinogen
( 1 1). Three extended studies in animals have been negative (32,33), including a 2-year ingestion study in rats (34). Although arecent investigation found initiating activity for bladder cancerwhen acrolein was administered intraperitoneally (35), com-plete carcinogenic activity could not be evaluated due to its
extreme toxicity. Acrolein is considered mutagenic (9, 36-38),presumably due to the formation of DNA adducts; in aqueoussolution, acrolein reacts with deoxyguanosine to produce two
major isomers of the hydroxy- 1 ,N2-propanodeoxyguanosineadduct and the 7,8-cyclic guanine adduct (Refs. 39-41 ; Fig.IB). Because ofthe toxicity ofacrolein (42), investigators haveincorporated 1 ,N2-propanodeoxyguanosine2 into shuttle vectors
2 l.N2-Propanodeoxyguanosine has been used as a model because the hydroxy-
I ,N2-propanodeoxyguanosine adduct is unstable under conditions used for oh-
godeoxynucleotide synthesis.
Association for Cancer Research. by guest on October 8, 2020. Copyright 1998 Americanhttps://bloodcancerdiscov.aacrjournals.orgDownloaded from
402 p53 in Cyclophosphamide-linked Cancer
Table 3 Correlation of mutations, add uct sites, and DNA rep air rates
Patientno.”
.p53 mutation p53 WT
sequence’
Phosph oramide mustard
adducts”
DNA�
re airp
rateExon Codon Base change CSB5 Site’ Intensity
18 5 135 G:C-*A:T Yes ttGct! ttGca Weak -
16 6 188 G:C-sC:G No [caGacl1� caGac Strong -
13 6 193 A:T-’G:C Yes NA NA NA Slow”
16 6 196 G:C-’C:G Yes ccGag acGaa Weak’ Slow
I I 6 199 G:C-.A:T Yes aaGgaaat aaGgaGtt Intermediate -
5 7 230 G:C-sA:T No ItgGta]5 aaGgtt Strong -
8 7 241 A:T-’T:A Yes NA NA NA -
10 8 Splice site G:C-sA:T Yes taGtg taGtt Weak -
6 8 279 G:C-sA:T Yes ctGgg ctGag Strong Slow’
“ Ordered sequentially by codon number.
S CSB, coding strand bias: NA, not applicable.
‘ Sequence is given in the 5’-’3’ direction. and the capital ‘G” represents the sites of mutation or adduction.
‘I 4-Hydroperoxycyclophosphamide (4-HC( adduction sites were taken from Bubley et al. (25); the 4-HC adduction sites are the same as those for phosphoramide mustard
(G. J. Bubley. personal communication).
� DNA repair rates for mutated codons were reported by Tornaletti and Pfeifer (30). -. not available.I Mutations at codons I 35 and 188 both match the GNC sequence pattern for interstrand cross-linking, where �‘N” is any nucleotide. For codon 135, the target guanine
on the opposite strand has 80% homology with an intermediate adduction site; therefore, this location is favorable for mutation because it has both intermediate and weakadduction sites in a GNC pattern.
A. Brackets indicate the sequence of the non-coding strand which contains the guanine residue. the presumed site of adduction.
‘, Although the mutated nucleotide is not a target for phosphoramide mustard adduction. codon 193 is a slow spot for DNA repair.
‘ The codon 196 mutation in patient 16 has only 60% homology with a weak adduction site, but that could be plausibly compensated by slow repair (30).
) Codon 279 is a potential mutation hotspot since it is a strong adduction site, and a slow spot for DNA repair is nearby in codon 278 (30).
(reviewed in Refs. 39 and 43) to evaluate acrolein-associated
mutations. In both bacteria and mammalian cells, the predom-
inant (75-90%) bp substitution is G:C-�T:A transversions (44,45), followed by G:C-*A:T transitions (10-25% of total mu-tations). Although the absence of G:C-�T:A transversions, thefingerprint of acrolein (44-46), in our series suggests a minimalrole for this metabolite in cyclophosphamide-associated bladder
cancer, further study in a larger number of cases is needed.
Summary and Implications. Our report provides the firstcorrelation between the location of carcinogen-DNA adductsand a characteristic spectrum of p53 mutations in cyclophos-
phamide-associated bladder cancer. These findings support anew paradigm (31, 47) for chemical carcinogenesis in which
the distribution of DNA adducts can be linked with an observedpattern of mutations. Further descriptions of specific configu-
rations of carcinogen-DNA adducts will facilitate the interpre-tation of complex p.53 mutation spectra, providing new insightsinto cancer etiology. Our findings suggest that phosphoramidemustard may be the primary mutagenic metabolite of cyclo-phosphamide in iatrogenic bladder cancer. If confirmed in a
larger series, these new results imply that chemoprotectantagents that bind nitrogen mustards (48) might be considered toameliorate the risk of cyclophosphamide-associated bladdercancer. Amifostine, for example, has been shown to decreasemutagenesis by nitrogen mustard (49, 50), presumably by re-
ducing mustard-induced DNA cross-links (5 1). In contrast,although available sulfhydryl compounds may prevent cyclo-phosphamide-related hemorrhagic cystitis by binding acrolein,
their inability to enter most cell types likely makes them inef-fective in blocking phosphoramide mustard mutagenicity (re-
viewed in Ref. 52).Further study of the pathogenesis of bladder cancer fol-
lowing well-characterized exposures, such as cyclophospha-mide, tobacco, and schistosomiasis, will continue to provide va]-
uable insights into underlying molecular mechanisms. In addition,because bladder cancer is now the fifth most common malignancyin the United States, with an estimated 54,500 cases expected tooccur in 1997 (53), further understanding of these tumors is im-portant for the development of prevention strategies.
Acknowledgments
We are indebted to Virginia Hunter, Judith Anderson, Diana Wagner, and Carla
Van Hoesen for assistance in identifying additional cases; to Loretta Brown,
Sondra van den Belt, Robert Opplinger, Connie Mahoney, Lori Odle, and Nancy
Holt for support in data collection; to Diane Fuchs for administrative coordina-
tion; to Rebecca Albert for technical expertise; to Tracy S. McNeish for compiling
p53 mutations and exposures; and to the many hospitals and physicians who
allowed access to treatment records.
References
I . Travis, L. B., Curtis, R. E., Glimelius, B., Holowaty, E. J., van Leeuwen, F. E.,
Lynch, C. F., Hagenbeek, A., Stovall, M., Banks, P. M., Adami, J., Gospoda-
rowicz, M. K., Wacholder, S., Inskip, P. D., Tucker, M. A., and Boice, J. D., Jr.
Bladder and kidney cancer following cyclophosphamide therapy for non-
Hodgkin’s lymphoma. J. NatI. Cancer Inst., 87: 524-530, 1995.
2. Fraiser, L. H., Kanekal, S., and Kehrer, J. P. Cyclophosphamide toxicity.
Characterising and avoiding the problem. Drugs. 42: 781-795, 1991.
3. Fernandes, E. T., Manivel, J. C., Reddy. P. K., and Ercole, C. J. Cyclophos-
phamide associated bladder cancer-a highly aggressive disease: analysis of 12
cases. J. Urol., 156: 1931-1933, 1996.
4. Grochow. L. B., and Colvin, M. Clinical pharmacokinetics of cyclophospha-
mide. In: M. M. Ames, G. Powis, and J. S. Kovach (eds.), Pharmacokinetics ofAnticancer Agents in Humans, pp. 135-154. Amsterdam: Elsevier, 1983.
5. Anderson, D., Bishop, J. B., Garner, R. C., Ostrosky-Wegman, P., and Selby,
P. B. Cyclophosphamide: review of its mutagenicity for an assessment of poten-
tial germ cell risks. Mutat. Res., 330: 1 15-181, 1995.
6. Kallama, S., and Hemminki, K. Alkylation of guanosine by phosphoramide
mustard, chloromethine hydrochloride and chlorambucil. Ada Pharmacol. Toxi-
col.. 54: 214-220, 1984.
7. Povirk, L. F., and Shuker, D. E. DNA damage and mutagenesis induced by
nitrogen mustards. Mutat. Res., 318: 205-226, 1994.
8. Hemminki. K. DNA adducts of nitrogen mustards and ethylene imines. In: K.
Hemminki. A. Dipple. D. E. G. Shiker. F. F. Kadlubar. D. Segerback. and H.
Bartsch (eds.), DNA Adducts: Identification and Biological Significance. pp.
313-321. Lyon: IARC, 1994.
9. Curren, R. D., Yang, L. L., Conklin, P. M., Grafstrom, R. C.. and Harris, C. C.
Mutagenesis of xeroderma pigmentosum fibroblasts by acrolein. Mutat. Res.,
209: 17-22, 1988.
10. Wilson, V. L., Foiles, P. G., Chung. F. L., Povey, A. C., Frank, A. A., and
Hams. C. C. Detection of acrolein and crotonaldehyde DNA adducts in culturedhuman cells and canine peripheral blood lymphocytes by 32P-postlabeling and
nucleotide chromatography. Carcinogenesis (Lond.), 12: 1483-1490, 1991.
Association for Cancer Research. by guest on October 8, 2020. Copyright 1998 Americanhttps://bloodcancerdiscov.aacrjournals.orgDownloaded from
Cancer Epidemiology, Biomarkers & Prevention 403
1 1. IARC Working Group June. Acrolein. In: IARC Working Group (ed), IARC
Monographs on the Evaluation ofthe Carcinogenic Risk ofChemicals to Humans,
pp. 133-161. Lyon: IARC, 1985.
12. Pedersen-Bjergaard, J., Ersboll, J., Hansen, V. L., Sorensen, B. L., Christ-
offersen, K., Hou-Jensen, K., Nssen, N. I., Knudsen, J. B., and Hansen, M. M.
Carcinoma of the urinary bladder after treatment with cyclophosphamide for
non-Hodgkin’s lymphoma. N. EngI. J. Med., 3/8: 1028-1032, 1988.
13. Talar-Williams, C., Hijazi, Y. M., Walther, M. M., Linehan, W. M., Halla-
han, C. W., Lubensky, I., Kerr, G. S., Hoffman, G. S., Fauci, A. S., and Sneller,
M. C. Cyclophosphamide-induced cystitis and bladder cancer in patients with
Wegener granulomatosis. Ann. Intern. Med., 124: 477-484, 1996.
14. Cox, P. J. Cyclophosphamide cystitis-identification of acrolein as the caus-
ative agent. Biochem. Pharmacol., 28: 2045-2049, 1979.
15. Reznikoff, C. A., Belair, C. D., Yeager, T. R., Savelieva, E., Blelloch, R. H.,
Puthenveettil, J. A., and Cuthill, S. A molecular genetic model of human bladder
cancer pathogenesis. Semin. Oncol., 23: 571-584, 1996.
16. Spruck, C. H., Rideout, W. M., Olumi, A. F., Ohneseit, P. F., Yang, A. S.,
Tsai, Y. C., Nichols, P. W., Horn, T., Hermann, G. G., Steven, K., Ross, R. K..
Yu, M. C., and Jones, P. A. Distinct pattern of p53 mutations in bladder cancer:relationship to tobacco usage. Cancer Res., 53: 1 162-1 166, 1993.
17. Warren, W., Biggs, P. J., el-Bar, M., Ghoneim, M. A., Stratton, M. R., and
Venitt, S. Mutations in the p53 gene in schistosomal bladder cancer: a study of
92 tumours from Egyptian patients and a comparison between mutational spectra
from schistosomal and non-schistosomal urothelial tumours. Carcinogenesis(Land.)., 16: 1181-1189, 1995.
18. Travis, L. B., Curtis, R. E., Glimelius, B., Holowaty, E., van Leeuwen, F. E.,
Lynch, C. F., Adami, J., Gospodarowicz, M., Wacholder. S., and lnskip. P.
Second cancers among long-term survivors of non-Hodgkin’s lymphoma. J. NatI.
Cancer. Inst., 85: 1932-1937, 1993.
19. DeBenedetti, V. M. G., Travis, L. B., Welsh, J. A., van Leeuwen, F. E.,
Stovall, M., Clarke, E. A., Boice, J. D., Jr., and Bennett, W. P. p53 mutations inlung cancer following radiation therapy for Hodgkin’s disease. Cancer Epidemiol.
Biomark. Prey., 5: 93-98, 1996.
20. Cariello, N. F., Piegorsch, W. W., Adams, W. T., and Skopek, T. R. Corn-
puter program for the analysis of mutational spectra: application to p53 mutations.
Carcinogenesis (Lond.), 15: 2281-2285, 1994.
21. Adams, W. T., and Skopek, T. R. Statistical test for the comparison of
samples from mutational spectra. J. Mol. Biol., 194: 391-396, 1987.
22. Lunec, J., Challen, C., Wright, C., Mellon, K., and Neal, D. E. c-erbB-2
amplification and identical p53 mutations in concomitant transitional carcinomas
of renal pelvis and urinary bladder. Lancet. 339: 439-440, 1992.
23. Oda, T., Tsuda, H., Scarpa, A., Sakamoto, M., and Hirohashi, S. Mutation
pattern of the p53 gene as a diagnostic marker for multiple hepatocellular
carcinoma. Cancer Res., 52: 3674-3678, 1992.
24. Taylor, J. A., Li, Y., He, M., Mason, T., Mettlin, C., Vogler, W. J., May-
garden. S., and Liu, E. p53 mutations in bladder tumors from arylamine-exposed
workers. Cancer Rca., 56: 294-298, 1996.
25. Bubley, G. J., Ogata, G. K., Dupuis, N. P., and Teicher, B. A. Detection of
sequence-specific antitumor alkylating agent DNA damage from cells treated in
culture and from a patient. Cancer Res., 54: 6325-6329, 1994.
26. Greene, M. H., Harris, E. L., Gershenson, D. M., Malkasian, G. D., Melton,
L. J., Dembo, A. J., Bennett, J. M., Moloney, W. C., and Boice, J. D., Jr.
Melphalan may be a more potent leukemogen than cyclophosphamide. Ann.
Intern. Med., /05: 360-367, 1994.
27. Kaldor, J. M., Day, N. E., Pettersson, F., Clarke, E. A., Pedersen, D.,
Mehnert, W., Bell, J., Host, H., Prior, P., and Karjalainen, S. Leukemia following
chemotherapy for ovarian cancer [see comments]. N. EngI. J. Med., 322: 1-6,
1990.
28. Bohr, V. A., Phillips, D. H., and Hanawalt, P. C. Heterogeneous DNA
damage and repair in the mammalian genome. Cancer Res., 47: 6426-6436.
1987.
29. Ford, J. M., Lommel. L., and Hanawalt, P. C. Preferential repair of ultraviolet
light-induced DNA damage in the transcribed strand of the human p53 gene. Mol.
Carcinog., 10: 105-109, 1994.
30. Tomaletti, S., and Pfeifer, G. P. Slow repair of pyrimidine dimers at p53
mutation hotspots in skin cancer. Science (Washington DC), 263: 1436-1438.
1994.
31. Denissenko. M. F., Pao, A.. Tang, M. S.. and Pfeifer. G. P. Preferential
formation of benzo(a)pyrene adducts at lung cancer mutational hotspots in p53.
Science (Washington DC), 274: 430-432, 1996.
32. Feron, V. J., and Kruysse. A. Effects of exposure to acrolein vapor in
hamsters simultaneously treated with benzo(a)pyrene or diethylnitrosamine. J.
Toxicol. Environ. Health. 3: 379-394. 1977.
33. Steiner, P. E., Steele. R., and Koch, F. C. The possible carcinogenicity of
overcooked meats. heated cholesterol, acrolein, and heated sesame oil. Cancer
Res., 33: 100-107, 1943.
34. Parent, R. A., Caravello. H. E.. and Long, J. E. Two-year toxicity and
carcinogenicity study of acrolein in rats. J. AppI. Toxicol.. /2: 131-139. 1992.
35. Cohen. S. M.. Garland, E. M., St. John. M.. Okamura. T., and Smith. R. A.
Acrolein initiates rat urinary bladder carcinogenesis. Cancer Res.. 52: 3577-358 I.
1992.
36. Bignami, M.. Cardamone, G., and Comba, V. A. Relationship between
chemical structure and mutagenic activity in some pesticides. The use of Sa!,no-
nella rvplsimurium and Aspergillus nidulans. Mutat. Res., 46: 243-244. 1977.
37. Vogel. E. W., and Nivard. M. J. Performance of 181 chemicals in a I)ro-
sophila assay predominantly monitoring interchromosomal mitotic recombina-
tion. Mutagenesis. 8: 57-81, 1993.
38. Dypbukt. J. M., Atzori, L., Edman, C. C.. and Grafstrom. R. C. Thiol status
and cytopathological effects of acrolein in normal and xeroderma pigmentosum
skin tibroblasts. Carcinogenesis (Lond.). 14: 975-980, 1993.
39. Mamett, L. J. DNA adducts of a,/3-unsaturated aldehydes and dicarbonyl
compounds. IARC Sci. Publ., /25: 151-163. 1994.
40. Chung, F-L., and Hecht, S. S. Formation of cyclic l,N2-adducts by reaction
of deoxyguanosine with a-acetoxy-N-nitrosopyrrolidine. 4-(carbethoxynitrosansi-
no)butanal, or crotonaldehyde. Cancer Res., 43: I 230-1 235. 1983.
41. Chung, F-L., Young. R.. and Hecht. S. S. Formation of cyclic l.N2-propa-nodeoxyguanosine adducts in DNA upon reaction with acrolein or crotonalde-
hyde. Cancer Res., 44: 990-995. 1984.
42. Parent, R. A., Caravello, H. E., and Harbell. J. W. Gene mutation assay of
acrolein in the CHO/HGPRT test system. J. AppI. Toxicol., 1/: 91-95. 1991.
43. Grollman, A. P., and Shihutani. S. Mutagenic specificity of chemical car-
cinogens as determined by studies of single DNA adducts. In: K. Ilemminki. A.
Dipple, D. E. G. Shuker, F. F. Kadlubar, D. Segerback. and H. Bartsch (eds.).
DNA Adducts: Identification and Biological Significance. pp. 385-397. Lyon:
IARC, 1994.
44. Moriya, M., Zhang. W.. Johnson, F.. and Grollman, A. P. Mutagenic potency
of exocyclic DNA adducts: marked differences between E.cc/,erichia coli and
simian kidney cells.Proc. NatI. Acad. Sci. USA, 91: 1 1899-1 903. 1994.
45. Hashim, M. F., and Mamett, L. J. Sequence-dependent induction of base pair
substitutions and frameshifts by propanodeoxyguanosine during in vitro DNA
replication. J. Biol. Chem.. 27/: 9160-9165. 1996.
46. Burcham, P. C.. and Mamett, L. J. Site-specific mutagenesis by a propan-
odeoxyguanosine adductcamed on an M13 genome. J. Biol. Chern.. 269: 28844-28850, 1994.
47. Denissenko, M. F.. Chen, J. X., Tang, M. S.. and Pfeifer. G. P. Cytosine
methylation determines hot spots of DNA damage in the human p53 gene. Proc.Natl. Acad. Sci. USA, 94: 3893-3898. 1997.
48. Capizzi, R. L. Amifostine: the preclinical basis for broad-spectrum selective
cytoprotection of normal tissues from cytotoxic therapies. Semin. Oncol.. 23:
2-17, 1996.
49. Nagy. B., and Grdina. D. J. Protective effects of 2-[(aminopropyl)aminoleth-
anethiol against bleomycin and nitrogen mustard-induced mutagenicity in V79
cells. Int. J. Radiat. Oncol. Biol. Phys.. 12: 1475-1478. 1986.
50. Kataoka, Y., Pemn. J., Hunter, N.. Milas, L., and Grdina, D. J. Antimutagenic
effects of amifostine: clinical implications. Semin. Oncol.. 23: 53-57. 1996.
51. DeNeve. W. J., Everett. C. K.. Suminski, J. E.. and Valeriotc. F. A. Influence
of WR2721 on DNA cross-linking by nitrogen mustard in normal mouse bone
marrow and leukemia cells in vito. Cancer Res.. 48: 60()2-6(X)5. 1985.
52. Goren, M. P. Oral mesna: a review. Semin. Oncol., 19: 65-71, 1992.
53. Parker. S. L.. Tong. T.. Bolden, S. A., and Wingo. P. A. Cancer Statistics1997. CA-A Cancer J. for Clinicians. 47: 5-27. 1997.
54. Hollstein, M., Shomer, B., Greenblatt, M., Soussi, T.. Hovig. E.. Montesano.
R., and Hams, C. C. Somatic point mutations in the p53 gene of human tumors
and cell lines: updated compilation. Nucleic Acids. Res., 24: 141-146, 1996.
Association for Cancer Research. by guest on October 8, 2020. Copyright 1998 Americanhttps://bloodcancerdiscov.aacrjournals.orgDownloaded from
1998;7:397-403. Cancer Epidemiol Biomarkers Prev M A Khan, L B Travis, C F Lynch, et al. p53 mutations in cyclophosphamide-associated bladder cancer.
Updated version
http://cebp.aacrjournals.org/content/7/5/397
Access the most recent version of this article at:
E-mail alerts related to this article or journal.Sign up to receive free email-alerts
Subscriptions
Reprints and
To order reprints of this article or to subscribe to the journal, contact the AACR Publications
Permissions
Rightslink site. Click on "Request Permissions" which will take you to the Copyright Clearance Center's (CCC)
.http://cebp.aacrjournals.org/content/7/5/397To request permission to re-use all or part of this article, use this link
Association for Cancer Research. by guest on October 8, 2020. Copyright 1998 Americanhttps://bloodcancerdiscov.aacrjournals.orgDownloaded from